The defect in Fas mRNA expression in MRL/lpr mice is associated with insertion of the retrotransposon, ETn.

Chu, Jia Li; Drappa, Jörn; Parnassa, Andrew; Elkon, Keith B.

doi:10.1084/jem.178.2.723

Cited by 230 publications

(113 citation statements)

References 31 publications

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“…Fas expression also was detected on a small proportion of GR-1 Ϫ PEC in B6 mice and GR-1 Ϫ and GR-1 lo PEC in B6/gld mice. Figure 1C shows that in B6/lpr mice, GR-1 hi inflammatory PEC do not express significant levels of Fas, as was expected because the lpr mutation reduces Fas expression to 10% or less of normal levels [2,[43][44][45].…”

Section: Fas Expression On Gr-1 Hi Inflammatory Neutrophilssupporting

confidence: 62%

Fas ligand (gld)- and Fas (lpr)-deficient mice do not show alterations in the extravasation or apoptosis of inflammatory neutrophils

Fecho

Cohen

1998

Journal of Leukocyte Biology

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Apoptosis of neutrophils plays a critical role in the resolution of acute inflammation. Neutrophils from human peripheral blood express Fas (CD95) and are sensitive to Fas ligand (FasL)/Fasmediated apoptosis. Mice carrying spontaneous mutations in the genes for fas ligand (B6/gld) or fas (B6/lpr) were used to assess the role of FasL/Fas in the kinetics and magnitude of neutrophil extravasation to the thioglycolate (TG)-inflamed peritoneum and in the spontaneous apoptosis of TGelicited neutrophils. The results showed that TG-elicited neutrophils (defined by flow cytometry as GR-1/Ly-6G hi cells) from normal (B6) and B6/ gld mice, but not from the Fas-deficient B6/lpr mice, express high levels of Fas. The TG-elicited neutrophil response began at 2 h, peaked at 4 h, and subsided by 24-48 h after TG administration in all three strains. However, the response was more prolonged in B6 mice, such that B6/gld and B6/lpr mice had fewer neutrophils at 6 h after TG administration than did B6 mice. Further studies showed that 4 h TG-elicited neutrophils from B6, B6/gld and B6/lpr mice undergo apoptosis in vitro at similar rates (as assessed through flow cytometry by the decrease in forward angle light-scatter and externalization of phosphatidylserine (PS; as detected by Annexin V-FITC) that occur as neutrophils undergo apoptosis). Fas expression was downregulated on apoptotic neutrophils in conjunction with maximal PS externalization and decreased forward angle light-scatter. Collectively, these findings suggest that FasL/Fas-mediated apoptosis is not essential in regulating the lifespan of neutrophils during an acute inflammatory response. The abbreviated inflammatory response observed in FasL/Fasdeficient mice is likely to be a secondary effect of the gld/lpr autoimmune/lymphoproliferative syndrome, and not a direct effect of FasL/Fas on the ability of inflammatory neutrophils to undergo apoptosis.

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Section: Fas Expression On Gr-1 Hi Inflammatory Neutrophilssupporting

confidence: 62%

Fas ligand (gld)- and Fas (lpr)-deficient mice do not show alterations in the extravasation or apoptosis of inflammatory neutrophils

Fecho

Cohen

1998

Journal of Leukocyte Biology

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“…That is, in addition to the association between genetic defects in Fas or Fas ligand and autoimmunity in mice (40)(41)(42)(43)(44)(45)(46)(47) and humans (48)(49)(50)(51), non-Fas-based abnormalities may play paramount roles in the pathogenesis and/or perpetuation of SLE.…”

Section: Discussionmentioning

confidence: 99%

Impaired nonrestricted cytolytic activity in systemic lupus erythematosus

Stohl

Elliott

et al. 1997

Arthritis & Rheumatism

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Objective. To determine the cytolytic effector pathway involved in impaired generation of nonrestricted cytolytic activity in systemic lupus erythemato- sus (SLE).Methods. Peripheral blood mononuclear cells (PBMC) from normal subjects and SLE patients were stimulated in vitro with anti-CD3 monoclonal antibody (MAb) and interleukin-2 to promote the generation of nonrestricted cytolytic activity. On day 13 of culture, the PBMC were assayed for cytolytic activity against FasDaudi cells and Fas+ Jurkat cells. The effects on cytotoxicity of calcium chelation, antagonist anti-Fas MAb, tumor necrosis factor (TNF) a and P, and ATP were measured. Intracellular perforin expression was determined by intracellular staining, and perforin messenger RNA levels were determined by quantitative competitive reverse transcription-polymerase chain reaction.Results. We demonstrated the existence of a cytolytic pathway that is independent of Fas, TNFa, TNFP, and ATP, but is dependent upon extracellular calcium. Despite its calcium dependence, this pathway is associated with low-to-undetectable levels of perforin.Conclusion. Impaired generation of nonrestricted ~-cytolytic activity in SLE is likely due to decreased activity of this Fas-, TNFa-, TNFP-, ATP-independent pathway associated with very low levels of perforin.

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“…A 1-kb cDNA probe encoding the FasR was produced from MRL/+ + thymus as described previously (11). To obtain cDNA probes encoding the FasL from rat (8) Northern Blot Analysis.…”

Section: Mice Mrl/ipr (Mr~l/mentioning

confidence: 99%

Massive upregulation of the Fas ligand in lpr and gld mice: implications for Fas regulation and the graft-versus-host disease-like wasting syndrome.

Chu

Ramos

Rosendorff

et al. 1995

The Journal of Experimental Medicine

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119

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The increased FasL expression is most likely due to repeated antigenic stimulation of T cells that cannot undergo apoptosis through the Fas pathway. Cell Culture and Subset Isolation. Single cell suspensions were prepared from the thymus, spleen, lymph nodes and, in some cases, bone marrow from different strains of mice. To induce expression of FasL, splenic T cells were activated by Con A 2 #g/ml and Ib2 (20 ng/ml) (8). The cells were cultured at 37~ in a humidified atmosphere in 5% CO2 at a density of 106 cells/ml in RPMI 1640 containing 10% FCS and 50 #M 2-ME. After 2 d in culture, the cells were further stimulated by PMA (10 ng/ml) and ionomycin (500 ng/ml) for 4 h. A toxic shock syndrome (TSST)-reactive T cell line (>99% CD4 § isolated from splenic T cells from an MRL/+ + mouse was kindly provided by Drs. S. Friedman and J. Tumang, Hospital for Special Surgery. Materials and Methods Mice. MRL/Ipr (MR~L/MpJCell subsets were isolated from the enlarged lymph nodes of 4-5-mo-old Ipr mice by negative selection. To obtain an enriched population of CD4-, CD8-double negative (DN) T cells, CD4+ and CD8 § single positive (SP) T cells were depleted by incubation of total lymph node cells with a cocktail of anti-CD4 and anti-CD8 mAb for 45 min at 4~ followed by incubation with guinea pig complement (Cedarlane Laboratories, Inc., Hornby, Canada) for I h at 37~ Residual SP T and B cells were removed by magnetic beads (Dynal, Oslo, Norway) coated with sheep anti-rat Ig. SP lymph node T cells were enriched by negative selection. DN T cells coated with the anti-B220 mAb as well as B cells 393 J. Exp.

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The defect in Fas mRNA expression in MRL/lpr mice is associated with insertion of the retrotransposon, ETn.

Cited by 230 publications

References 31 publications

Fas ligand (gld)- and Fas (lpr)-deficient mice do not show alterations in the extravasation or apoptosis of inflammatory neutrophils

Fas ligand (gld)- and Fas (lpr)-deficient mice do not show alterations in the extravasation or apoptosis of inflammatory neutrophils

Impaired nonrestricted cytolytic activity in systemic lupus erythematosus

Massive upregulation of the Fas ligand in lpr and gld mice: implications for Fas regulation and the graft-versus-host disease-like wasting syndrome.

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